TECHNICAL FIELD
[0001] This patent document relates to nanotechnologies.
BACKGROUND
[0002] Nanotechnology provides techniques or processes for fabricating structures, devices, and systems with features at a molecular or atomic scale, e.g., structures in a range of one to hundreds of nanometers in some applications. For example, nano-scale devices can be configured to sizes within one hundred to ten thousand times smaller than human cells, e.g., similar in size to some large biological molecules (biomolecules) such as enzymes and receptors. Nano-sized materials used to create a nanostructure, nanodevice, or a nanosystem that can exhibit various unique properties that are not present in the same materials scaled at larger dimensions and such unique properties can be exploited for a wide range of applications.
US 2010/0055170 A1 discloses nanocapsules comprising a silica shell including pore channels and a metal core within a cavity of the silica shell.
US4671909A1 discloses hollow microspheres comprising shells including macropores. The pore structure allows impregnation with enzymes.
US 2005/0244322 A1 discloses mesoporous core-silica shell particles.
Li, J., et al., Soft Matter, 2010, 6, 542-550, discloses a method of fabricating microcapsules via a layer-by-layer approach.
Yu, A., et al., Adv. Mater, 2005, 17, 1737-1741, discloses a method of preparing enzyme loaded biocompatible microcapsules.
Li, G., et al., Chem. Mater, 2010, 22, 1309-1317, discloses a nanoparticle delivery device with either 2 silica shells and a silica core or hollow double-layered PMAA shelled-microcapsules loaded with DOX.
SUMMARY
[0003] Techniques and devices are described for fabricating and implementing nanostructures or nanoparticles that include a hollow core and sealable holes.
[0004] In one aspect of the disclosed invention, a method is defined to fabricate a nanoparticle device comprising combining a core particle with one or more masking particles to form a template, wherein the one or more masking particles bind to the core particle and cover one or more regions of the surface of the core particle, each of the one or more regions corresponding to a surface area formed between each of the one or more masking particles and the core particle;forming a layer over the template, wherein the layer forms over the surface of the core particle excluding the covered one or more regions;removing the template to produce a shell structure having one or more holes extending between an interior region that is hollow and an external surface, the one or more holes having a size on the external surface substantially that of the surface area and distributed on the shell structure at the one or more regions;loading a substance into the interior region of the shell structure through the one or more holes, wherein the substance includes a macromolecule; and forming an outer layer over the shell structure, wherein the outer layer seals the one or more holes of the shell structure and encloses the substance within the interior region, wherein the one or more holes are mesopores with a size ranging from 2 nm to 50 nm, and the mesopores are sealed with a nanoporous shell material; and wherein the outer layer includes pores with a size less than 2 nm to allow molecules smaller than 2 nm to diffuse in and out but prevent macromolecules from entering and leaving.
[0005] In another aspect of the invention, defined is a nanoparticle device carrying a substance comprising:a shell structure including at least two layers including an internal layer and an external layer,wherein the substance includes a macromolecule;wherein the internal layer encloses a hollow interior region comprising the substance in the hollow region;wherein the internal layer includes one or more holes penetrating said internal layer, the one or more holes having a diameter larger than the diameter of the macromolecule,wherein the one or more holes are mesopores with a size ranging from 2 nm to 50 nm, and the mesopores are sealed with a nanoporous shell material,wherein the external layer is formed around the internal layer and includes pores with a size less than 2 nm to allow substances smaller than 2 nm to diffuse in and out but prevent macromolecules from entering or leaving;wherein the substance and the internal layer are such that the substance is capable of passing through the one or more holes of the internal layer; and wherein the substance and the external layer are such that the substance is incapable of passing through the external layer.
[0006] The subject matter described in this patent document can be implemented in specific ways that provide one or more of the following features. For example, the disclosed nano- and micro-structures can include nanoparticles having sealable holes to a hollowed interior that can encapsulate other substances contained inside the hollow region. The exemplary hollow nanoparticles with sealable holes further include pores that permit transport of selected particles or substances, while not permitting transport of the encapsulated substances. Exemplary methods to fabricate the disclosed nanoparticles (e.g., the exemplary hollow porous nanoparticles (HPNPs)) are described offering precise control and flexibility over the size and permeability of the nanoparticles, e.g., using a variety of materials. The described nanostructures include exemplary features including, for example, a high characteristic surface area and hollow interior capable for loading substances, which can enable implementations in a broad range of applications, e.g., including nanomedicine, catalysis, optics, waste removal, among many other applications. The disclosed nanostructures can be applied to medical diagnostics, monitoring and therapy, e.g., such as prodrug-enzyme therapy, enzyme or gene delivery and sensor applications. Exemplary nanomedicine applications can include controlled release of drugs, biological molecules and chemicals, immuno-isolation and protection of biomolecules and biologically active species, building blocks for photonic crystals, and removal of waste substances. For example, one or more macromolecules or macromolecular system(s) is encapsulated in an exemplary HPNP and be sealed afterwards, e.g., forming a sealed hollow porous nanoparticle (SHPNP), after which the exemplary macromolecule(s) can still be in communication with the environment, e.g., via small molecules that can traffic in and out through the pores of the SHPNP.
[0007] In an example of an application using the disclosed technology, the exemplary macromolecule encapsulated in the exemplary SHPNP can be a molecule capable of signaling the occurrence of a particular event such as pH change. When pH changes in the environment, the pH change can be detected by the exemplary encapsulated macromolecule, e.g., because ions can move through the pores of the exemplary SHPNP. For example, in this configuration, the exemplary macromolecule used to detect the pH change is not introduced to the environment and therefore does not activate any immune response. Similarly, the exemplary SHPNPs can be used for different applications, e.g., in which the encapsulated structure is an enzyme. For example, an enzyme can be encapsulated in an SHPNP and be used to activate a drug molecule, e.g., which it binds to that would be otherwise deactivated. The exemplary enzyme is protected inside the exemplary SHPNP from the immune system, and the outside of the exemplary SHPNP can be conjugated to targeting agents to enable specific binding to a targeted site within the environment. Once the exemplary SHPNP having the encapsulated enzyme is delivered to the target site (e.g., tumor), a deactivated drug can be introduced into the blood flow of the organism (e.g., since the drug is deactivated, there is no limitation of drug dose). Also, for example, since the drug is a small particle, it can diffuse to many regions associated with the target site. However, the drug can be activated only at the region having the exemplary enzyme-encapsulated SHPNP, e.g., which can be targeted to that particular site or region. Therefore, in this example, the drug is only activated at the target site, e.g., by moving through the SHPNP pores and interacting with the encapsulated enzyme (e.g., activating the drug), and then moving out through the SHPNP pores to treat the tumor. For example, drug delivery via the disclosed nanoparticles can be used to provide stabilization, extended circulation, and targeting. In other examples, the encapsulated load can include proteins responsible for activating a certain mechanism, other nanoparticles, and/or toxic substances, e.g., protected from the biological environment that the exemplary SHPNPs are deployed.
BRIEF DESCRIPTION OF THE DRAWINGS
[0008]
FIGS. 1A-1C show schematic diagrams illustrating an exemplary nanoparticle synthesis protocol.
FIGS. 2A-2B show process diagrams of an exemplary nanoparticle synthesis protocol.
FIG. 3 shows exemplary transmission electron microscopy (TEM) images showing the structural properties of exemplary hollow porous nanoparticles.
FIG. 4 shows scanning electron micrograph (SEM) images exhibiting degrees of freedom of the synthesis on exemplary hollow nanoparticle features.
FIGS. 5A and 5B show an SEM image of exemplary aggregates and resultant hollow porous nanoparticles.
FIG. 5C shows SEM images of exemplary unsealed and sealed hollow porous nanoparticles.
FIG. 6 shows an illustration of an exemplary implementation using the disclosed sealed hollow porous nanoparticles.
FIGS. 7A and 7B show SEM images of exemplary hollow porous nanoparticles.
FIGS. 8A-8I show electron micrographs of exemplary hollow porous silica nanoparticles.
FIGS. 9A-9D show schematic illustrations of an exemplary fabrication process to create sealed hollow porous nanoparticles.
FIGS. 10A and 10B show data plots showing activity of sealed hollow porous nanoparticles of the disclosed technology.
FIGS. 10C-10E show electron micrographs showing exemplary nanoparticles.
FIG. 11 shows an image demonstrating in vivo activity in the disclosed technology.
FIG. 12 shows a data plot showing activity of free Bacillus cereus penicillinase with and without incubation with proteinase-K.
FIG. 13 shows a data plot showing activity of free Renilla reniformis luciferase with and without incubation with proteinase-K.
FIG. 14 shows a data plot showing a standard curve of Bacillus cereus penicillinase activity.
FIG. 15 shows a data plot showing activity of different concentrations of free Bacillus cereus penicillinase compared to that encapsulated within sealed hollow porous nanoparticles.
FIG. 16 shows a data plot showing a standard curve of Renilla reniformis luciferase activity.
FIG. 17 shows a data plot showing activity of different concentrations of Renilla reniformis luciferase compared to that encapsulated within sealed hollow porous nanoparticles.
FIGS. 18A and 18B show schematic diagrams illustrating an exemplary metallic nanoparticle synthesis protocol.
FIG. 18C shows an image of exemplary hollow porous gold nanoparticles.
FIG. 19 shows schematic diagrams illustrating an exemplary nanoparticle synthesis protocol.
FIG. 20 shows schematic diagrams illustrating an exemplary nanoparticle synthesis protocol.
[0009] Like reference symbols and designations in the various drawings indicate like elements.
DETAILED DESCRIPTION
[0010] Nanostructures such as nanoparticles can be used to carry chemical or biological substances (e.g., drugs) as loads and be deployed for delivery of the loaded substances in a variety of environments, including biological environments such as within an organism. For example, nanostructure carriers deployed in an
in vivo environment can themselves trigger an immune response and/or cause toxicity issues, e.g. which can be due to the nanoparticle carrier material and/or the loaded substance material. In some cases, drug delivery systems via nanoparticles can require modification of the loaded substance, which can reduce the desired function of the loaded substance.
[0011] Techniques and devices are described for fabricating and implementing nanoparticles that include a hollow core and sealable holes.
[0012] The disclosed nanoparticles and nanoparticle systems include a hollow nanoparticle-based carrier platform that is capable of encapsulating and protecting substances within an interior region of the nanoparticle, through sealable holes. For example, the disclosed nanoparticle-based carrier platform can include hollow porous nanoparticles that can enclose a molecular load such that it is hidden from the immune system within its hollow core, while allowing controlled interaction of the enclosed load within the desired environment, e.g., via pores on the surface that lead to the interior region of the nanoparticle. For example, the exemplary hollow porous nanoparticles can themselves be biocompatible, but encase a non-biocompatible load. For example, implementation using the disclosed nanoparticles and nanoparticle systems in some applications can eliminate the need for modifying a payload substance, prevent triggering of an undesired immune response when deployed in an organism, allow flexible surface functionalization of the nanoparticle (e.g., for targeting), or extend circulation lifetime of the nanoparticles independent of the loaded substance(s). Also for example, the disclosed nanoparticles and nanoparticle systems can include a hollow non-porous nanoparticle-based carrier platform that is capable of encapsulating and protecting substances within the interior region of the nanoparticle through sealable holes and release the encapsulated substances into an environment that the nanoparticle is deployed, e.g., in which the sealable holes can dissolve and release the load in the deployed environment. In other examples, the disclosed nanoparticles and nanoparticle systems can include a hollow nanoparticle-based carrier platform that is capable of encapsulating and protecting substances within the interior region of the nanoparticle through sealable holes and release the encapsulated substances into an environment that the nanoparticle is deployed, e.g., in the nanoparticle can dissolve and release the load in the deployed environment.
[0013] In one aspect, the disclosed technology includes fabrication techniques that can be used to create nano-scale structures (e.g., such as nano-cage or nano-shell particles) having sealable holes and small pores, each of controllable sizes, e.g., in which the structure can encapsulate other substances contained within an interior region. Described are fabrication methods that can produce hollow porous nanoparticle (HPNPs) having holes configured to a controllable size, e.g., which can allow entry of other substances or particles (e.g., macromolecules) within its hollow interior. The described fabrication methods include techniques to seal the holes of the HPNPs, e.g., forming sealed hollow porous nanoparticles (SHPNPs), which can enclose the loaded substances or particles within the SHPNPs. For example, to fabricate HPNPs, a core particle is used as a starting template material, e.g., which can be in the form of any shape, including a sphere, conc, rod, rectangular solid, tube, among others. Masking particles can bind to the external surface of the template material, e.g., by intermolecular interactions. A porous shell can be formed by applying a coating material around the template material forming a core shell nanoparticle. Afterwards, the core and bound masking particles can be removed, e.g., by dissolution or calcination or other similar methods, in which the porous shell remains. Implementation of this process can form hollow porous nanoparticles, and other molecules can be encapsulated inside the interior of the produced nanoparticle. For example, the described fabrication methods can include techniques to load and seal the holes completely, e.g., once the exemplary macromolecules are encapsulated inside, enabling the porous shell particle as a loaded carrier. For example, the hole size can be adjusted independent of the size of the nanoparticle size. For example, the described fabrication methods can include techniques to independently adjust the pore size.
[0014] Exemplary template-based techniques are described that can use a variety of materials (e.g., including polymers, ceramics, and metals) to prepare HPNPs with monodisperse sizes, e.g., ranging from several tens of nanometers to micrometers in core particle diameter. The exemplary template-based techniques can be used to produce surface holes of controllable sizes along the hollow particle shell, e.g., ranging from a few nanometers to tens or hundreds of nanometers in hole diameter. The described fabrication techniques can provide independent control of the permeability of HPNPs. For example, permeability of the HPNPs can be configured by controlling the porosity of the shell material, e.g., producing pores of sizes that can range from a few to several nanometers. For example, nanometer pore sizes can result in relatively low permeability of large macromolecules diffusion into / out of the HPNPs, e.g., preventing enzymes, proteins or larger biologically active materials to diffuse through the HPNP while still permitting smaller substances to diffuse through the pores. For example, exemplary implementations using silica and gold HPNPs are described demonstrating precise control of particle size and surface porosity. The described fabrication techniques can be modified to produce HPNPs of different materials, e.g., including, but not limited to, calcium-based nanoparticles such as calcium phosphate or calcium coated particles, iron oxide nanoparticles, among other materials. For example, fabricating HPNPs of different materials can provide engineering of the properties of the HPNPs that can be suitable for particular desired applications.
[0015] The exemplary techniques can include colloidal templating reactions on surfaces with different chemical and physical properties. For example, a layer of shell material is grown over a colloidal particle template with parts of the surface blocked by smaller masking colloidal particles. Subsequently, the template and masking particles are removed by methods such as, for example, calcination and/or dissolution, to leave the hollow particle with open holes on the surface. For example, the overall size of the particle is determined by the template particle. For example, the diameter of the holes can be adjusted by varying the size of the masking particles, and the number of holes on the particle surface can be controlled by the relative molar concentration of template and masking particles.
[0016] The disclosed technology includes several protocols for fabricating the nanoparticles with hollow core, porous surface and sealable holes. FIGS. 1A-1C show schematic diagrams illustrating one exemplary nanoparticle synthesis according to the invention.
[0017] FIG. 1A shows an example of a process
110 in which masking particles
115 are mixed together with one or more core or template particles
111. For example, the masking particles
115 can be nanoparticles configured to have a surface charge, e.g., a negative surface charge. Also, for example, the masking particles
115 can include particles with a functionalized external surface
116, e.g., having a surface charge. For example, the exemplary masking particles
115 can be polystyrene nanoparticles, and the exemplary functionalized surface
116 can be a carboxylated-functional layer. For example, the template particle
111 can be a nanoparticle configured to have a surface charge, e.g., a positive surface charge, of opposite polarity to the surface charge of the masking particles
115. Also, for example, the template particle
111 can include a particle with a functionalized external surface
112. For example, the exemplary template particle
111 can be a polystyrene nanoparticle, and the exemplary functionalized surface
112 can be an amine-functional layer. For example, once the exemplary carboxylated masking particles
115 and aminated template particle
111 are mixed, the carboxylated particles
115 can bind to the aminated template particle
111.
[0018] FIG. 1A also shows an example of a process
120 of binding of the masking particles
115 with the carboxylated functionalized surface
116 to the aminated functionalized surface
112 of the template particle
111, e.g., by electrostatic interactions. For example, when the exemplary carboxylated particles
115 have a negatively charged surface, they repel negative ions and prevent sol-gel reaction on their surfaces, e.g., blocking some positively charged regions of the outer surface of the exemplary aminated template particle
111. In other examples, the process
120 can include binding the masking particles
115 to the surface
112 of the template particle
111 by other particle attraction means, e.g., including, but not limited to, hydrogen bonding, covalent bonding, magnetic attraction, hydrophobic interactions, etc.
[0019] FIG. 1A further shows an example of a process
130 of adding a layer
131 to the masking particles
115 - template particle
111 complex. For example, sol-gel reagents can be added to the solutions containing the masking particles
115 bound to the template particles
111. Exemplary sol-gel reactions can occur only in the positively charged regions along the surface
112 of the template particle
111, e.g., the regions that are not covered or blocked by the masking particles
115. The process
130 covers the exposed surface of the template particle
111 with the coating
131 while not covering locations where the masking particles
115 are present. For example, the coating
131 can be a porous material. For example, the layer
131 can be of a material (e.g., silica) such that the process
130 can result in a porous layer forming on the surface of the template particle
111. For example, addition of sol-gel reactants in the process
130 can initiate silica growth, e.g., rooted from the amino groups of the exemplary aminated functionalized surface
112. Also exemplified, but not claimed is where the coating
131 can be a non-porous material. In some examples, the process
130 can include adding the layer
131 to the masking particles
115 - template particle
111 complex by other means, e.g., including, but not limited to, material based exclusivity, or redox chemistry that forms the layer
131 only on the surface of one particle (e.g., the template particle
111) and not the surface of the other particle(s) (e.g., the masking particles
115), among other techniques. Exemplary materials used for the coating can include porous or or degradable materials (e.g., that can dissolve or degrade in certain environments or under particular conditions or by an exemplary trigger, e.g., conditions and/or trigger including pH, temperature, pressure, molecular interaction, or other conditions and/or triggers).
[0020] In addition, FIG. 1A shows an example of a process
140 of forming a hollow nanoparticle, e.g., by removing the template particle
111 and the masking particles
115. For example, once the layer
131 is formed with the desired thickness, the template particle
111 and masking particles
115 are removed, e.g., by various methods including dissolving them by solvents, calcination, melting, or burning, or a combination of these or other similar methods. For example, the process
140 can include introducing dimethylformamide (DMF), acetone, or other solvent and/or heat to the layer-covered masking particles
115 - template particle
111 complex. Implementation of the process
140 yields an HPNP that includes empty or hollowed porous shell
141 with holes
145 and an empty or hollowed interior
142. In some non-claimed examples, the process
140 can be implemented to form a hollow non-porous nanoparticle, e.g., by removing the template particle
111 and the masking particles
115. For example, a hollow non-porous nanoparticle can be formed by implementing the process
130 using an exemplary non-porous material as the coating
131. In such examples, the exemplary shell
141 is a hollowed non-porous shell.
[0021] Once the exemplary HPNPs are created, they are loaded with macromolecules and sealed to encapsulate the loaded substances.
[0022] FIG. 1B shows an example of a process
150 for loading load particles
151 into the hollow interior region
142 of the shell structure
141. For example, a solution of shell structures (e.g., HPNPs) can be loaded with the load substances by adding a high concentration solution of the load substances to the solution of the shell structures. The process
150 can be implemented by one of several methods. For example, the load particles
151 can diffuse into the shell structures
141 through the holes
145. In other examples, the load particles
151 can enter the interior region
142 of the shell structures
141 through their holes
145 by non-diffusion means, e.g., including electrophoretic forces. The process
150 can be implemented using various types of materials as the load, e.g., including, but not limited to, drugs, biodegradable macromolecules, pH sensitive molecules, enzymes, hormones, and/or other proteins, glycoproteins, glycolipids, carbohydrates, lipids, nucleic acid, aptamer, metals, polymers, and ceramic particles, for various applications.
[0023] After loading the shell structures
141 with the load particles
151, the holes
145 are sealed. FIG. 1C shows processes
160 and
170 showing forming a sealed hollow porous nanoparticle
175, e.g., by sealing the holes
145 of the exemplary HPNP
141 that encloses the load particles
151 within the hollow interior region
142. In this example, the holes
145 are sealed with a further layer of a porous material (e.g., silica) shown as layer
171. In other non-claimed examples, the holes
145 can be sealed with a further layer of a non-porous material (e.g., a metal layer or other non-porous material), which can also be represented by the layer
171.
[0024] The process
160 can include partially covering the holes
145 with a layer
161 (e.g., a large positively charged polymer such as poly-L-lysine (PLL)). For example, the PLL polymer can create a mesh like structure over the surface of the exemplary HPNP
141 and the holes
145. The process
170 includes sealing the load particles
151 within the exemplary HPNP
141 to form a sealed hollow porous nanoparticle
175. For example, the process
170 can include forming a layer
171 over the exemplary PLL-covered HPNP
141. For example, further addition of sol-gel reactants can create another layer (e.g., the layer
171) on top of the initial layer (e.g., the layer
161) covering the holes
145, e.g., by nucleation sites that are on the exemplary PLL polymer, thereby forming the exemplary SHPNP
175. For example, the exemplary load particles
151 can be permanently sealed and enclosed inside the exemplary SHPNP
175. In some examples, the process
170 can be implemented to form the exemplary sealed hollow porous nanoparticle
175 without implementing the process
160, e.g., by forming a layer
171 directly over the exemplary shell structure
141. In some non-claimed examples, a sealed hollow non-porous nanoparticle can be formed by implementing the processes
160 and
170 using an exemplary non-porous material as the coating
131. In such examples, the exemplary shell
141 is a hollowed non-porous shell (e.g., with the load particles
151 inside the hollow interior region
142) that can be covered with the layer
161 (e.g., a large positively charged material, forming a mesh-like structure over the surface of the exemplary shell structure
141 and the holes
145), and the holes
145 can be sealed (e.g., enclosing the load particles
151 within the exemplary shell structure
141) by forming the layer
171 over the exemplary layer
161-covered shell structure
141, thereby forming the exemplary sealed hollow nanoparticle
175. In this example, the exemplary sealed hollow nanoparticle
175 can include a non-porous layer
141 and a porous layer
171, e.g., in which small particles or substances can traffic in and out of the exemplary nanoparticle
175. Also in such examples, the process
170 can be implemented to form the exemplary sealed hollow nanoparticle
175 without implementing the process
160, e.g., by forming a layer
171 directly over the exemplary shell structure
141 (e.g., loaded with the load particles
151 inside the hollow interior region
142).
[0025] For example, the process
170 can include determining a material for the layer
171 can be based on a desired application. In some non-claimed examples, the exemplary sealed hollow nanoparticle
175 can include a porous layer
141 and a porous layer
171. In other non-claimed examples, the exemplary sealed hollow nanoparticle
175 can include a non-porous layer
141 and a porous layer
171. In other examples, the exemplary sealed hollow nanoparticle
175 can include a porous layer
141 and a non-porous layer
171. And in other non-claimed examples, the exemplary sealed hollow nanoparticle
175 can include a non-porous layer
141 and a non-porous layer
171.
[0026] The load particles
151 are macromolecules.
[0027] The exemplary fabrication process depicted in FIG. 1A can be implemented using polystyrene nanoparticles with amino functional groups as the exemplary template particles and polystyrene nanoparticles with carboxyl functional groups as the exemplary masking particles. For example, amino functional groups are positively charged and can facilitate the chemistry used in the exemplary fabrication process. In some examples, exemplary sol-gel reagents require a positively charged nucleation site, which can be provided by the aminated functionalized surface. Fabrication of exemplary HPNPs can be implemented using materials such as vesicular solution, colloids, emulsion droplets and polymers as templates for forming a layer of target material or its precursor. For example, the exemplary fabrication process can be implemented using silicic acid is used as a precursor. For example, silicic acid gives negatively charged silicon-containing ions to the solution. These exemplary negatively charged ions are attracted by the positively charged template nanoparticle surface. For example, silica can be selected as a coating material over the masked template surface; e.g., properties of silica can include adjustable porosity, thermal and mechanical stability, low density, high specific surface area, and biocompatibility and biodegradability, which can be important properties in medical- and biological-based applications.
[0028] Exemplary silica HPNPs were fabricated for use in exemplary implementations of the disclosed technology. For example, amine-functionalized polystyrene nanoparticles (APNPs) can be used as the template for nucleating growth of the nanoporous silica sol-gel network. For example, tetramethoxysilane (TMOS) is hydrolyzed in aqueous solution to give silicic acid, which acts as a precursor for the polycondensation reaction on the particle surface. Exemplary chemical reactions below describe the initial stages of the polycondensation reaction of silicic acid resulting in the growth of silica layer.
Si(OCH3)4 +
4 H2O →
Si(OH)4 +
4 HOCH3 +
4 OH-
Si(OH)4 +
OH- →
Si(OH)3O- +
H2O
Si(OH)4 +
Si(OH)3O- →
(HO)3 Si-O-Si
(OH)3 +
OH-
[0029] For example, the exemplary fabrication process can include mixing APNPs with carboxyl-functionalized polystyrene latex nanoparticles (CPNPs) in an aqueous solution (e.g., illustrated in the process
110 of FIG. 1A). The exemplary APNPs and CPNPs can aggregate together, e.g., due to electrostatic interaction of functional groups (e.g., illustrated in the process
120 of FIG. 1A). For example, the exemplary particles with oppositely charged surface functional groups attract each other in solution. For example, the amine functionalized surface creates a more efficient nucleation site for base-catalyzed silica gel growth compared to the acidic carboxyl-functionalized surface. At the point of contact, CPNPs serve as a negatively charged nanomask for the sol-gel reaction on the particle surface. The exemplary fabrication process can include adding silane to the solution to be hydrolyzed and give silicic acid, e.g., which acts as a precursor to the silica layer. For example, basic amine groups on the APNPs can template silica gel growth efficiently, whereas acidic carboxyl groups on the CPNPs can mask the reaction at point of contact with the APNPs (e.g., illustrated in the process
130 of FIG. 1A). The exemplary fabrication process can include removing the APNPs and CPNPs through, for example, calcination or dissolution. Once the silica layer is formed with the desired thickness, the polystyrene particles are removed by dissolution or calcination leaving the silica HPNP structure (e.g., illustrated in the process
140 of FIG. 1A). In some examples, the exemplary fabrication process can include resuspending and dispersing the HPNPs in water using vortex mixing and gentle sonication. For example, the final particle diameter after calcination can be approximately 85% of the diameter of the initial 500 nm template APNPs, which may be related to partial dehydration of the silica gel hydroxyl groups during heating or extraction with anhydrous solvents.
[0030] For example, the fabrication process can be implemented to produce silica shell particles (e.g., HPNP
141 in FIG. 1A, and SHPNP
175 in FIG. 1C) having pores that allow small molecules to get through. However, the large molecule load (e.g., load particles
151 shown in FIG. 1C) cannot get through the holes, and is therefore sealed within the particle. There can be other variations of this exemplary fabrication technique (described in FIGS. 1A-1C) that can be based on the desired application. For example, the HPNP can be formed of metal (e.g., such as gold), or there can be multiple or multiple varying layers of different materials that form the HPNP, e.g., such as a first internal layer of metal and a second external layer of polymer (e.g., silica). The size of the particle can be determined by the size of the template particle, and the sizes of the holes can be determined by the sizes of the blocking or masking particles. The size of the disclosed hollow porous nanoparticle and the size of its holes can be configured independent of each other. In addition, the porosity of the HPNP can be configured independent of the size of the HPNP and the size of its holes.
[0031] FIGS. 2A-2B show process diagrams of the synthesis protocol to produce hollow porous nanoparticles and sealed hollow porous nanoparticles. FIG. 2A shows a process diagram
200 that includes a process
201 to bind nanomask particles to a core particle, a process
202 to form a layer over the nanomask-bound core particle, and a process
203 to form a hollow porous shell particle including holes, e.g., by removing the nanomask particles and the core particle. FIG. 2B shows a process diagram
210 that includes a process
211 to load macromolecules into the hollow porous shell particle through the holes and a process
212 to seal the holes of the hollow porous shell particle to enclose the loaded molecules or other substances within.
[0032] The exemplary fabrication methods of the disclosed technology provide precise control of nanoporosity and particle diameter independently. For example, the exemplary fabrication methods can be applied to the broad range of materials accessible through sol-gel synthesis routes. In addition, the exemplary fabrication methods can be applied for different chemistries including gold and redox based chemistries, e.g., expanding the suitability of HPNPs to a broad range of applications.
[0033] Exemplary fabrication methods were employed using, e.g., tetramethoxysilane (TMOS) solution, which was obtained from Aldrich-Sigma Ltd. Exemplary chemicals were used as received. For example, amine functionalized polystyrene beads were obtained from Polysciences, Inc. and carboxyl-functionalized polystyrene latex particles were obtained from Life Technologies, Inc.
[0034] Exemplary implementations of the disclosed technology included the preparation of hollow porous silica nanospheres. For example, a 50 µL template particle solution was mixed with the corresponding amount of masking particle solution to prepare the desired ratio of particle concentrations. The resultant mixture was shaken overnight and 1000 µL of anhydrous ethanol was added to the solution. In order to generate the silica precursor and initiate the silica growth, 1 µL of tetramethoxysilane was added to the solution. The mixture was shaken overnight, and the suspended particles were collected by centrifugation (e.g., 5 min at 14000 rpm), washed with deionized water a few times and dried in vacuum overnight on a coverslide. To remove the organic compounds, a coverslide carrying the nanoparticle powder was placed over a hot plate and calcined overnight at 450 °C. The calcined powder was transferred to a tube and suspended in water (e.g., 50 µL) and dispersed by gentle sonication.
[0035] Exemplary implementations of the disclosed technology included the preparation of sealed hollow porous silica nanospheres. For example, 4 µL of 10 mg/mL enzyme solution was added to 50 µL of the exemplary hollow porous silica nanospheres solution and incubated overnight. The exemplary solution was diluted with 1000 µL phosphate buffered saline and 50 µL 0.1% poly-L-lysine with a molecular weight of 150-300 kDa. For example, the exemplary solution can be diluted to prevent aggregation. TMOS was added to 1 mM HCl in 74:500 volume ratio and mixed for a few minutes to make silicic acid solution. 25 µL of the exemplary silicic acid solution was added to the above porous silica nanospheres solution immediately after the dilution and shaken for 1 hr, e.g., in order to generate sealed hollow porous silica nanospheres. Later, suspended sealed hollow porous silica nanospheres were collected with centrifugation (e.g., 5 min at 14000 rpm) and washed several times with water. Samples were exposed to proteinase-K enzyme overnight at a concentration of 0.1 mg/mL in IX phosphate buffered saline (PBS) solution at 37 °C, followed by removal of proteinase-K by successive washing again by IX PBS by centrifugation (e.g., 5 min at 14000 rpm). The described protocol can be used for encapsulation of payload substances. For example, the payload substances utilized in the exemplary implementations included penicillinase and
Renilla reniformis luciferase, e.g., encapsulated within exemplary hollow porous silica nanospheres.
[0036] For example, penicillinase from
Bacillus cereus was obtained from Sigma-Aldrich Co., LLC. CCF2-AM was obtained from Life Technologies, Inc., San Diego, California, USA. Rabbit polyclonal biotinylated antibody was obtained from GeneTex, Inc., San Antonio, Texas, USA. All fluorescence intensities were measured on an Infinite 200 Pro, TECAN, Switzerland.
[0037] Exemplary implementations of the disclosed technology included the preparation of hollow silica nanospheres, in which a similar fabrication protocol to that of the described hollow porous silica nanospheres was implemented, except omitting nanomasks.
[0038] Exemplary implementations of the disclosed technology included the labeling of penicillinase with Cy5. For example, Cy5 maleimide was used as labeling agent for exemplary implementations demonstrating the described protocol. For example, 1 mg penicillinase was dissolved in 100 µL degassed PBS buffer at 10 mg/mL concentration. For example, thiol modifications were carried out under nitrogen in degassed solvents/buffers. The exemplary solution was left at room temperature for around 30 min. About 100 molar excess of TCEP was added to the exemplary solution. The vial was flushed with nitrogen gas, capped and mixed thoroughly. This reaction was incubated at room temperature for 10 min. 100 µg Cy5 maleimide was dissolved in 2 µL dimethylformamide (DMF) and added to the enzyme solution. The vial was again flushed with nitrogen, capped and mixed thoroughly. This solution was incubated at room temperature for 2 hr while being mixed every 30 min. Finally, the reaction was left overnight at 2-8 °C. Later, unbound dye was removed by a desalting column with a molecular weight cut-off at 7 kDa.
[0039] The activity is measured in 100% normal mouse serum as the initial rate of increase of the ratio of blue fluorescence (447 nm) to green fluorescence (520 nm) with excitation at 409 nm.
[0040] The amount of enzyme loading (e.g., the exemplary Cy5 labeled penicillinase) was detected by measuring fluorescence intensity at 620 nm excitation and 665 nm emission.
[0041] Antibody binding was measured in the following exemplary manner. For example, anti-penicillinase was functionalized with biotin groups. Alexa 488 dye with streptavidin was added to all samples followed by successive washing. Fluorescence intensity measurements were performed at 480 nm excitation and 530 nm emission.
[0042] Exemplary implementations of the disclosed technology included
in vivo activity measurements, which were prepared and performed in the following exemplary manner. For example, BALB/c mice were used in the exemplary implementations. For example, one mouse was injected with 100 µL of
Renilla reniformis luciferase (RenLuc) enzyme encapsulated sealed hollow porous silica nanospheres solution intramuscularly. The exemplary sealed hollow porous silica nanospheres were suspended in IX phosphate buffered saline (PBS) with a concentration of 5.68×10
12 particles/mL. For example, the other mouse was injected with 100 µL 8 µg/mL concentration of free RenLuc intramuscularly. Free RenLuc was suspended in IX PBS. 5 minutes later, 10 µg benzyl-coelenterazine was administered intravenously in the lateral tail vein of each mouse. 10 µg benzyl-coelenterazine was dissolved in 95% ethanol and diluted with IX PBS to 10% final concentration of alcohol. Mice were by isoflurane and luminescence intensities were measured from each mouse following intravenous injections with an exposure of 2 sec.
[0043] Exemplary implementations of the disclosed technology included the characterization of nanostructures. For example, SEM measurements were conducted on a FEI/Philips XL30 FEG ESEM, and ultra high resolution (UHR) SEM measurements were performed on FEI SFEG UHR SEM with acceleration voltages of 10 kV (e.g., at the UC San Diego, Calit2 Nano3 Facility). TEM images were obtained with the use of a FEI Technai Sphera 200 kV (e.g., UC San Diego, Cryo-Electron Microscopy). A Hitachi HD-2000 instrument was used for scanning transmission electron microscope (STEM) images operating at 200 kV. IVIS Imaging System 200 Series from Xenogen Corporation, Alameda, California (e.g., at UC San Diego, Moores Cancer Center) was used for
in vivo luminescence measurements.
[0044] Exemplary implementations performed are described that demonstrate precise control of the particle diameter, hole diameter, and hole concentration of exemplary silica hollow porous nanoparticles using the fabrication techniques of the disclosed technology. For example, the robustness and flexibility of the disclosed fabrication techniques offer the ability to implement the fabricated nanoparticles in a variety of common and unique applications in many fields.
[0045] High resolution electron micrographs are presented in FIG. 3 that reveal the structure of the generated holes. FIG. 3 shows exemplary transmission electron microscopy (TEM) images
301, 302, 303, and
304 exhibiting the structural properties of exemplary HPNPs. For example, the exemplary HPNPs can be generated by using 500 nm APNPs as template particles and 100 nm CPNPs as the masking or blocking particles. The image
301 shows a close-up view of the surface features of an exemplary HPNP, e.g., taken by secondary electron mode of scanning transmission electron microscope (STEM), which revealed the formation of 30 ± 10 nm holes formed at the point of contact of the template and masking nanoparticles. The image
302 shows a TEM image of exemplary HPNPs displaying the hole structure and the thickness of the silica shell. The image
303 shows an SEM micrograph, e.g., taken with ultra high resolution mode, which shows the open-hole structure throughout the shell and the thickness of the shell from an interior perspective. The image
304 shows a wide field electron micrograph, e.g., taken by the transmission mode of STEM, which shows the monodispersity and evenness of exemplary uniform HPNPs. For example, the images of FIG. 3 show that silica formation is completely prevented around the point of contact between two particles and that the curvature of the masking CPNP surface is reflected by the surface topography of the resultant particle. For example, the exemplary synthesis using 500 nm APNP templates and TMOS to APNP weight ratio of 3:1 can result in silica shells with a thickness of 25 nm. This thickness can be related to yielding stable particles.
[0046] FIG. 4 shows scanning electron micrograph (SEM) images
401, 402, 403, and
404 exhibiting degrees of freedom of the synthesis on exemplary HPNP features. The image
401 shows an exemplary HPNP surface exhibiting -25-30 number of holes, e.g., by preparation using 500 nm APNP templating particles and 100 nm CPNP masking particles with a APNP-to-CPNP number ratio of 1:30. The image
402 shows an exemplary HPNP surface exhibiting ∼10-15 number of holes, e.g., by preparation using the same templating and masking particles with a APNP-to-CPNP number ratio of 1:15 The image
403 shows a micrograph of HPNPs obtained using 500 nm APNPs and 40 nm CPNP taken by SEM. The image
404 shows an SEM image of HPNPs generated using 200 nm APNPs and 40 nm CPNP. The inset image
405 shows a higher resolution close-up TEM micrograph of these exemplary particles, e.g., where the exemplary arrows indicate the holes on the particle surface. The exemplary scale bar shown in the images
401,
402,
403, and
404 represents 100 nm, and the exemplary scale bar shown in the inset image
405 represents 50 nm.
[0047] The disclosed fabrication procedures can include multiple degrees of freedom in producing the HPNPs. For example, the exemplary fabrication process can include control of the number of holes on the surface (e.g., exemplified in the image
402), diameter of the holes (e.g., exemplified in the image
403) and overall particle size (e.g., exemplified in the image
404). For example, the average number of holes on the surface can be controlled by the relative molar concentration of the APNPs and CPNPs. SEM micrographs in the images
401 and
402 show the hole distribution on the surface when the APNP to CPNP molar ratios in solution are 1:30 and 1:15, respectively. The exemplary molar ratios of APNPs to CPNPs can result in ∼25-30 holes per particle for the 1:30 ratio and ∼10-15 holes per particle for the 1:15 ratio.
[0048] For example, the size of the holes created on the surface (e.g., hole diameter) can be adjusted by selecting masking CPNPs with different diameters independently of the overall diameter of the HPNPs. The exemplary hole size of the HPNPs shown in the image
401 include 30 ± 6 nm diameter holes, e.g., created using CPNPs with a 100 nm diameter on 500 nm APNP. The exemplary hole size of the HPNPs shown in the image
402 include 20 ± 3 nm diameter holes, e.g., created using CPNPs with a 60 nm diameter on 500 nm APNP. Exemplary CPNPs can be configured with diameters of ∼20 nm to produce HPNPs with holes having a diameter of a few nanometers.
[0049] For example, the overall size of the HPNP depends on the template particle size. Exemplary APNPs can be configured in a wide range of sizes to prepare HPNPs, e.g., in ranges of ∼30 nm to several micrometers. For example, HPNPs created by 500 nm APNP templates can shrink by about 15% upon template removal, e.g., resulting in HPNPs with diameters of 430 nm (as shown in the exemplary HPNP in the image
401). However, for example, the percent of shrinkage is not constant with changing APNP template size; in exemplary implementations, HPNPs fabricated by using 200 nm APNPs and 40 nm CPNPs resulted in an overall particle size of 150 nm corresponding to a shrinking by about 25% after calcination (as shown in the exemplary HPNP in the image
404). For example, increased shrinking may be explained by the higher relative volume ratio of the dehydrated hydroxyl groups to the total silica volume when using a smaller particle. Exemplary template and masking particle combinations resulted in holes about 25-35% of the diameter of the initial masking particles, e.g., decreasing slightly with smaller dimensions. For example, the slight decrease for smaller nanomasks may be related to increasing surface curvature resulting in a smaller point of contact. For example, a closer and higher resolution TEM micrograph shown in the inset image
405 of the 150 nm HPNPs includes arrows indicating the holes on the particle surface. For example, the diameter of the holes formed on the HPNPs fabricated using the 200 nm APNP / 40 nm CPNP pair resulted in 12 ± 2 nm.
[0050] FIG. 5A shows an SEM image
510 of exemplary aggregates formed by 500 nm APNPs as template particles and 100 nm CPNPs as the masking or blocking particles. FIG. 5B shows an SEM image
520 of exemplary resultant HPNPs using the particle framework in the image
510. The exemplary scale bar shown in images
510 and
520 represents 200 nm.
[0051] FIG. 5C shows SEM images of exemplary unsealed HPNPs (shown in image
531) and sealed hollow porous nanoparticles (SHPNPs) (shown in image
532). The exemplary scale bar shown in FIG. 5C represents 100 nm.
[0052] The disclosed porous nanoparticles can be implemented in variety of applications, including very unique applications that may not be possible with any other method. For example, enzymes with non-human origin can be useful in a variety of therapeutic applications. However, immune responses, as well as proteolysis within endocytic organelles and organs of metabolic clearance, are generated against these foreign proteins and can hinder their therapeutic functionality.
[0053] In another aspect, the disclosed technology includes a porous shell based nano carrier platform that encapsulates and protect a foreign macromolecular cargo from antibodies, proteases, and other biomolecules that may compromise the cargo's desired functionality. The described porous shell based nano carrier platform can also be referred to as HPNPs. The porous shell based nano carrier platform can include hollow spherical nanoshells including mesopores, 2 to 50 nm, that enable high-capacity loading of unmodified macromolecules, in which the loaded particles can be subsequently sealed with nanoporous material that still allows small molecules to easily diffuse in and out but prevents macromolecules from entering or leaving. The described sealed porous shell based nano carrier platform can also be referred to as SHPNPs.
[0054] The exemplary SHPNPs can be applied to
in vivo medical diagnostics, monitoring and therapy, e.g., such as enzyme-prodrug therapy, enzyme replacement therapy, therapies based on enzymatic depletion of tumor nutrients, and
in vivo biosensing. For example, since SHPNPs can be configured as thin hollow nanoshells, minimal inorganic mass is introduced while maximizing
in vivo loading capacity. For example, the disclosed SHPNPs can be implemented to prevent immune response against their foreign enzymatic cargos and protect them from proteolysis. The SHPNPs include nanopores, < 2nm diameter, on their surfaces for substrates to reach encapsulated macromolecules within the hollow core interior, interact with and be modified by the macromolecules, and diffuse out (as exemplified in FIG. 6).
[0055] FIG. 6 shows a schematic diagram
600 illustrating the exemplary implementation of the disclosed sealed hollow porous nanoparticles having loaded enzymatic cargo for use in an enzyme-prodrug therapeutic application. The diagram
600 shows a sealed hollow porous nanoparticle
611 that encloses enzymes
615 within its hollow interior for interaction with prodrug molecules
616, the interaction occurring inside the SHPNP
611. For example, the enclosed enzymes
615 are protected inside the SHPNP
611, e.g., from the immune system or other substances in the environment in which the SHPNP
611 is deployed. For example, since the particle surface is porous, prodrug molecules
616 can diffuse into the SHPNP
611 and subsequently interact with the enzymes
615, e.g., depicted as prodrug-enzyme complex
617. For example, the enzyme
615 can be used to activate the prodrug molecule
616, e.g., which is otherwise deactivated. The interaction between the enzyme
615 and the prodrug
616 at the prodrug-enzyme complex
617 can result in the formation of an activated drug
626. The activated drug
626 can diffuse out of the SHPNP
611 and subsequently interact with a target that the drug is designed to treat.
[0056] Exemplary implementations of the SHPNP
611 can include deployment into a living organism for therapeutic drug delivery. For example, the external surface of the SHPNP
611 can be conjugated to targeting agents, e.g., to enable specific binding to a targeted site within the environment. For example, once the SHPNP
611 having the encapsulated enzyme
615 is delivered to a target site (e.g., tumor), a deactivated drug (e.g., the prodrug
616) can be introduced into the blood flow of the organism. Although the prodrug
616 can be exposed to a multitude of regions within the organism, the prodrug
616 can be activated only at the region having the exemplary enzyme-encapsulated SHPNP
611, e.g., which can be targeted to that particular site or region. Therefore, in this example, the prodrug
616 is only activated at the target site, e.g., by moving through the pores into the SHPNP
611 and interacting with the encapsulated enzyme
615 (e.g., activating the prodrug
616), and after which the activated drug
626 moving out through the pores into the SHPNP
611 to treat the exemplary tumor.
[0057] The fabrication of the exemplary SHPNPs (e.g., illustrated in the diagram
600) are fabricated using the techniques previously described and shown in FIGS. 1A-1C, e.g., which include a high yield and scalable synthesis method that utilizes nanomasks preventing templating reaction on parts of the shell surface. For example, the described fabrication techniques lead to the formation of mesopores, 2 to 50 nm, in HPNPs and SHPNPs for efficient loading of macromolecules e.g., such as enzymes. For example, the non-claimed HPNPs can be made from a shell of nanoporous material with mesopores on the surface allowing large biomolecules to diffuse into the hollow interior volume of the particles. For example, once large molecules of interest are loaded, the mesopores can be sealed with a nanoporous shell material (e.g., the same material used to form the HPNPs), thereby forming loaded SHPNPs.
[0058] For example, the surface of exemplary SHPNPs can be further functionalized for targeting and improved circulation half-life. The exemplary further functionalization of the SHPNPs can eliminate the need for any modification of the loaded substances. For example, under these conditions, stealth SHPNPs can be delivered to a targeted region and allow continuous and controlled access of a substrate to interact with the enzyme cargo within the protected environment of the SHPNPs, e.g., making them an ideal therapeutic platform for
in vivo enzyme delivery for pro-drug therapies for diseases including cancer.
[0059] Exemplary SEM images of hollow porous nanoparticles are presented in FIGS. 7A and 7B, e.g., which demonstrate the implementation of the described HPNP synthesis techniques, e.g., previously described in FIG. 1A-1C. FIG. 7A shows an SEM image
710 of aggregated APNPs and CPNPs. For example, CPNPs are mixed with larger APNPs, and the CPNPs and APNPs having oppositely charged surface functional groups attract each other in solution causing aggregation. The image
710 demonstrates the framework for exemplary HPNP synthesis techniques showing 500 nm APNPs and 100 nm CPNPs. For example, the basic nature of the amine-functionalized surface can create a more efficient nucleation site for base-catalyzed silica gel growth compared to the acidic carboxyl-functionalized surface. For example, at the point of contact, CPNPs serve as negatively charged nanomasks for the sol-gel reaction on the particle surface. For example, once the silica layer is formed with the desired thickness, the polystyrene particles are removed leaving the silica hollow porous nanoparticle structure. FIG. 7B shows an SEM image
720 of silica hollow porous nanoparticles. For example, the final HPNP diameter after calcination is shown in the image
720 at about 85% of the diameter of the initial 500 nm template APNPs (as shown in the image
710), e.g., which may be related to partial dehydration of the silica gel hydroxyl groups during heating or extraction with anhydrous solvents. The exemplary scale bar represents 200 nm in the images
710 and
720.
[0060] Structural properties of the described hollow porous nanoparticles are shown in FIGS. 8A-8I. FIGS. 8A-8I include electron micrographs of silica HPNPs made from 500 nm templates and 100 nm nanomasks. FIG. 8A shows an electron micrograph
801 revealing the surface topography of an exemplary hollow porous nanoparticles taken with secondary electron mode of STEM. For example, the image
801 shows that silica formation is completely prevented around the point of contact between two particles and the curvature of the masking CPNP surface, which is reflected by the surface topography of the resultant particle. FIG. 8B shows a transmission electron micrograph
802 of an exemplary HPNP. For example, the exemplary synthesis technique using 500 nm APNP templates and TMOS to APNP weight ratio of 3:1 produced silica shells with a thickness of 25 nm. This exemplary thickness can yield stable particles in this size range. FIG. 8C shows a scanning electron microscope image
803 of an exemplary cracked HPNP showing the open-hole structure from an interior perspective. FIG. 8D shows an electron micrograph
804 taken with transmission mode of STEM showing the monodispersity of exemplary HPNPs.
[0061] The disclosed fabrication procedures can be applied to particles with different features in a wide range of sizes. For example, three degrees of freedom in the fabrication of HPNPs can include the number of holes on the surface, the diameter of the holes, and the overall particle size. FIG. 8E shows an SEM image
805 showing an exemplary HPNP formed by 500 nm templates and 100 nm nanomasks, e.g., with the particle number ratio of 1:30. FIG. 8F shows an SEM image
806 showing an exemplary HPNP formed by 500 nm templates and 100 nm nanomasks with the particle number ratio of 1:15. For example, the average number of holes on the surface is controlled by the relative molar concentration of the APNPs and CPNPs. SEM micrographs in FIGS. 8E and 8F show the hole distribution on the surface when the APNP to CPNP molar ratios in solution are 1:30 and 1:15, respectively. These ratios result in 25-30 holes per particle for the 1:30 ratio (e.g., shown in FIG. 8E) and 10-15 holes per particle for the 1:15 ratio (e.g., shown in FIG. 8F). FIG. 8G shows an SEM image
807 showing an exemplary HPNP formed by 500 nm templates and 60 nm nanomasks. For example, the size of the holes created on the surface can be adjusted by selecting masking CPNPs with different diameters independently of the overall diameter of the HPNP. The use of 100 nm masking CPNPs can produce holes of 30 ± 4 nm in diameter (e.g., shown in FIGS. 8E and 8F), and the use of 60 nm masking CPNPs can produce holes of 20 ± 3 nm in diameter at the point of contact (e.g., shown in FIG. 8G). Exemplary CPNPs can be used having a 20 nm in diameter, e.g., yielding holes down to several nanometers with high accuracy.
[0062] FIG. 8H shows an SEM image
808 showing an exemplary HPNP formed by 200 nm templates and 40 nm nanomasks. For example, the overall size of the HPNP can be configured based on the template particle size. The exemplary HPNPs created by 500 nm APNP templates were shown to reduce in diameter by about 15% upon template removal resulting in HPNPs with diameters of 430 nm (e.g., shown in FIGS. 8E-8G). However, the percent of shrinkage is not constant with changing APNP template size; e.g., exemplary HPNPs generated by using 200 nm APNPs and 40 nm CPNPs resulted in an overall particle size of 150 nm corresponding a shrinking about 25% after calcination (e.g., shown in FIG. 8H). For example, increased shrinking may be due to the higher relative volume ratio of the surface hydroxyl groups to the total silica volume when using a smaller particle. The exemplary scale bar represents 50 nm in the image
808.
[0063] Exemplary implementations performed showed that template and nanomask particle combinations resulted in holes (e.g., mesopores) about 25-35% of the diameter of the initial nanomasks, e.g., decreasing slightly with smaller dimensions. For example, the slight decrease for smaller nanomasks may be related to increasing surface curvature resulting in a smaller point of contact. FIG. 8I shows a TEM image
809 showing an exemplary HPNP of a 150 nm diameter. The exemplary arrows shown in the image
809 indicate holes on the surface. For example, the diameter of the holes was shown to be 12 ± 2 nm, and the exemplary HPNP was formed by 200 nm APNPs and 40 nm CPNPs. The exemplary scale bar represents 50 nm in the image
809.
[0064] FIGS. 9A-9D show schematic illustrations of an exemplary fabrication technique of SHPNPs. FIG. 9A shows a process
910 of producing an HPNP
911 including a hollow interior core
912 and holes
913 (e.g., mesopores) extending through the exterior shell of the HPNP
911 to the hollow interior core
912. For example, the HPNP
911 can include small pores that permit traffic of small molecules in and out of the HPNP
911. For example, the process
910 can include the implementation of the processes
110,
120,
130, and
140 to produce the HPNP
911. FIG. 9B shows a process
920 of loading enzymes
925 into the HPNP
911. For example, the process
920 can include adding a high concentration of a solution containing the enzymes
925 to a solution containing the HPNPs
911 (e.g., which can be in an HPNP suspension). For example, the process
920 can include the enzymes
925 diffusing into the hollow interior
912 of the HPNP
911 through the holes
913 by diffusion. For example, since the holes are relatively large compared to the enzymes, the enzymes
925 can freely diffuse into the structure quickly, equilibrating the concentration inside and outside of the HPNPs
911. In other examples, the process
920 can load the enzymes
925 into the hollow interior
912 of the HPNP
911 through the holes
913 by electrophoretic forces. FIG. 9C shows a process
930 of partially covering the holes
913 and the surface of the HPNP
911 with a layer
931. For example, the process
930 can include a depositing a large positively charged polymer such as PLL. For example, the layer
931 can be configured as a PLL polymer layer that can create a mesh like structure over the surface of the HPNP
911 and the holes
913. FIG. 9D shows a process
940 of sealing the enzymes
925 within the HPNP
911 to form a sealed hollow porous nanoparticle
945. For example, the process
940 can include forming a layer
941 over the layer-covered HPNP
911. For example, further addition of sol-gel reactants can create another layer (e.g., the layer
941) on top of the initial layer (e.g., the layer
931) covering the holes
913, e.g., by nucleation sites that are on the exemplary PLL polymer, thereby enclosing the enzymes
925 within the SHPNP
945.
[0065] For example, in the case of a silica HPNP, the surface of the HPNP
911 is negatively charged due to SiO
- groups. A positively charged polymer such as PLL can be added to adsorb to the particles' surface and change the surface charge to positive. Subsequently, TMOS can be added to grow a new layer of silica on the surface, e.g., closing the holes (e.g., mesopores) of the HPNP
911. This exemplary reaction can occur in near neutral buffer condition and does not damage the enzyme load. For example, once the mesopores are closed, the load is encapsulated within the SHPNP
945 and cannot escape. However, the load can still interact with small molecules in the surrounding environment via diffusion through nanopores.
[0066] This exemplary capability can be used to provide several benefits. For example, the exemplary enzyme load is hidden from the immune system, e.g., because antibodies are too large to pass through the nanopores to reach the enzyme. For example, the exemplary enzyme load is protected from the immune system and from digesting enzymes, e.g., such as proteases, while still remaining completely active. For example, the exemplary SHPNPs can be coated with passivating and targeting ligands without any chemical modification of the payload, e.g., the enzyme load, providing an effective strategy for
in vivo applications.
[0067] Exemplary implementations were performed to characterize the enzymatic activity and protection abilities of the disclosed SHPNPs. For example, penicillinase from
Bacillus cereus is a member of the family of beta-lactamases which catalyze the hydrolysis of the betalactam ring.
B. cereus penicillinase was utilized in exemplary characterization implementations of SHPNPs, e.g., because it can be considered a preferred beta-lactamase for enzyme-prodrug based therapies, and sensitive chromogenic and fluorogenic assays were available. For example, the latter used the substrate CCF2, which contains a coumarin linked to fluorescein via a cephalosporin group. For example, before cleavage by penicillinase, excitation of the coumarin at 409 nm causes efficient fluorescence resonance energy transfer (FRET) to fluorescein, resulting in green emission peaking around 520 nm. For example, penicillinase cleaves the cephalosporin group, separating fluorescein from coumarin and disrupting FRET, so that the same excitation produces blue 447 nm emission from coumarin. CCF2 is generally available as an acetoxymethyl (AM) ester, which rapidly reverts to CCF2 upon exposure to esterases in rodent plasma and serum as well as inside cells.
[0068] FIGS. 10A and 10B are exemplary data plots showing enzymatic activity of sealed hollow porous nanoparticles of the disclosed technology. FIG. 10A shows a data plot 1010 of the activity comparison for SHPNPs with encapsulated penicillinase and CCF2-AM as substrate in normal serum. For example, four exemplary samples were characterized, which included sample 1 of hollow nanoshells, sample 2 of HPNPs, sample 3 of sealed hollow nanoshells, and sample 4 of SHPNPs. All four of the exemplary samples were incubated with enzyme followed by successive washing with IX PBS and with proteinase-K again after successive washing with IX PBS. The exemplary sealing reaction was performed after enzyme incubation before washing for the exemplary samples 3 and 4. The data shown in the data plot
1010 demonstrates activity of penicillinase enzyme (e.g., MW = 28 kDa) encapsulated within the exemplary SHPNPs. All of the exemplary samples were exposed to proteinase-K, e.g., which can digests protein. Therefore, for example, sustained activity of the encapsulated enzyme after exposure to proteinase-K demonstrates the protection of the encapsulated enzyme against proteolysis by encapsulation in SHPNPs (as shown later in FIGS. 12 and 13).
[0069] For example, as shown in FIG. 10A, the data plot
1010 shows that the exemplary sample 1 and the exemplary sample 2 demonstrated no or little activity, which was expected after exposure to proteinase-K. For example, the data plot
1010 shows a 2-fold increase in activity of the exemplary sample 3 over the exemplary sample 1, e.g., which can be due to the protection provided by the second layer of silica over the enzymes stuck on the surface supporting the protective effect of the additional silica layer. However, a significant increase in activity was shown by the exemplary sample 4 of the SHPNPs. For example, the data plot
1010 shows a 10-fold activity increase of the SHPNPs over the exemplary sample 3, e.g., demonstrating that the increase is not due to the enzyme covering the surface but rather due to the enzyme molecules filling the hollow interior. The substantial difference shown between the exemplary HPNPs (of sample 2) and the exemplary SHPNPs (of sample 4) further supports this finding, e.g., since these two samples have undergone the same fabrication techniques except for the additional sealing process by the exemplary sample 4.
[0070] FIG. 10B shows a data plot
1020 of the activity comparison for polyclonal antibody binding against encapsulated penicillinase. The data plot
1020 includes exemplary red bars
1021 representing the fluorescence from Alexa 488 with streptavidin that can attach antibody molecules with biotin. The data plot
1020 includes exemplary blue bars
1022 representing the fluorescence from Cy5 labeled penicillinase. For example, three exemplary samples were characterized, which included sample 1 of empty SHPNPs, sample 2 of hollow silica shells in which penicillinase was adsorbed on the surface, sample 3 of SHPNPs with encapsulated penicillinase. For example, the exemplary samples 1 and 3 were incubated with proteinase-K to remove any enzyme that might have been stuck to the surface. All three exemplary samples were washed several times to remove unbound enzymes.
[0071] The exemplary data plot
1020 shown in FIG. 10B can be used to evaluate the antibody access to the enzyme encapsulated in exemplary SHPNPs. For example, the penicillinase was fluorescently labeled with Cy5, and its accessibility was probed with a rabbit polyclonal biotinylated antibody against penicillinase, e.g., detected by Alexa488-labeled streptavidin. The data plot
1020 shows that the measured intensity from exemplary samples 1 and 3 are comparable (e.g., within the standard error interval), e.g., indicating that the slight fluorescence coming from the exemplary sample 3 is not associated with antibodies, but rather from nonspecific adsorption of Alexa488-streptavidin. For example, the exemplary sample 2 showed around 5-fold higher intensity, e.g., demonstrating significant antibody binding to the enzyme molecules on the surface of the silica. For example, the data plot
1020 shows no fluorescence from the exemplary sample 1, e.g., which was expected due to lack of penicillinase. For example, the data plot
1020 shows no antibody binding to the exemplary sample 3, e.g., although it has the highest amount of penicillinase content, which establishes prevention of antibody access to the encapsulated enzyme within SHPNPs.
[0072] FIGS. 10C-10E are electron micrographs showing exemplary nanoparticles. FIG. 10C shows an image
1030 of exemplary 200 nm hollow non-mesoporous nanoshells. FIG. 10D shows an image
1040 of exemplary HPNPs formed by 200 nm templates and 40 nm nanomasks. FIG. 10E shows an image
1050 of exemplary SHPNPs formed by sealing HPNPs (produced by fabrication methods using 200 nm templates and 40 nm nanomasks). Exemplary scale bars represent 100 nm in the images
1030, 1040, and
1050.
[0073] FIG. 11 shows an image
1100 demonstrating
in vivo activity in BALB/c mice of
Renilla reniformis luciferase (RenLuc) enzyme. For example, the exemplary RenLuc enzyme was encapsulated in 200 nm SHPNPs in a similar manner as penicillinase was in the previous implementation, e.g., including shaving with proteinase-K to remove any surface-exposed RenLuc. The illuminated and luminescence pictures in the image
1100 were overlaid. For example, an exemplary BALB/c mouse
1101 (shown on the left of the image
1100) was injected intramuscularly with 100 µL of RenLuc enzyme encapsulated SHPNP solution at a concentration of 5.68×10
12 particles/mL, followed by lateral tail vein injection of 10 µg benzyl-coelenterazine after 5 minutes. As a control, an exemplary mouse
1102 (shown on the right of the image
1100) was injected intramuscularly with 100 µL of 8 µg/mK concentration of free RenLuc enzyme. Both exemplary injections demonstrated similar
in vitro activity (as shown later in FIGS. 16 and 17). For example, the data obtained in the image
1100 included an exemplary procedure in which 5 min after intramuscular injection, 10 µg benzyl-coelenterazine was administered intravenously in the lateral tail vein. Luminescence intensities were measured from each mouse 5 minutes after intravenous injections. Luminescence intensity from the mouse injected with RenLuc encapsulated SHPNPs was measured as 2.6×10
5 p/sec/cm
2/sr indicating localized activity of encapsulated enzymes within SHPNPs, whereas the intensity from the mouse injected with free RenLuc was below the detectable limit. For example, lack of luminescence from the latter may be mainly due to diffusion of free enzyme out of the injection site.
[0074] FIG. 12 shows a data plot
1200 showing activity plots of free
Bacillus cereus penicillinase with and without incubation with proteinase-K for 12 hours at 37 °C in IX normal mouse serum. For example, 5 µM CCF2-AM was used as substrate, and the activity was measured in 100% normal mouse serum as the initial rate of increase of the ratio of blue fluorescence (447 nm) to green fluorescence (520 nm) with excitation at 409 nm. The data plot
1200 includes a plotted data
1201 of free
Bacillus cereus penicillinase without incubation with proteinase-K and a plotted data
1202 of free
Bacillus cereus penicillinase with incubation with proteinase-K.
[0075] FIG. 13 shows a data plot
1300 showing activity plots of free
Renilla reniformis luciferase with and without incubation with proteinase-K for 12 hours at 37 °C in IX normal mouse serum. For example, each reaction was 100 µL in total containing 10 µg/mL benzyl-coelenterazine as substrate. The data plot
1300 includes a plotted data
1301 of free
Renilla reniformis luciferase with incubation with proteinase-K and a plotted data
1302 of free
Renilla reniformis luciferase without incubation with proteinase-K.
[0076] FIG. 14 shows a data plot
1400 showing a standard curve of
Bacillus cereus penicillinase activity. For example, initial rate of increase in absorbance in nitrocefin assay was represents the vertical axis of the data plot
1400.
[0077] FIG. 15 shows a data plot
1500 showing activity plots of different concentrations of free
Bacillus cereus penicillinase compared to
B. cereus penicillinase encapsulated within sealed hollow porous nanoparticles with a concentration of 1.42×10
12 particles/mL. For example, each reaction was 100 µL in total containing 250 µg/mL nitrocefin as substrate, and absorbance was measured at 486 nm. For example, the data plot
1500 shows penicillinase activity for concentrations including 0 mg/mL (curve
1501), 0.1 mg/mL (curve
1502), 0.02 mg/mL (curve 1503), 0.004 mg/mL (curve
1504), and 0.0008 mg/mL (curve
1505), and shows 1.42×10
12 SHPNPs/mL (curve
1506).
[0078] For example, the standard curve of free
B. cereus penicillinase (shown in the data plot
1400) compared to the measured activity of the
B. cereus penicillinase encapsulated within the SHPNPs corresponded to 4.58×10
-14 international units (IU) from a single 200 nm SHPNP, e.g., -50 enzyme molecules per particle based on a yield of HPNP synthesis is 100%. For example, during enzyme loading, HPNPs were initially incubated with 26.4 µM. For example, the assayed concentration of enzyme within a single SHPNP can correspond to 19.5 µM, e.g., resulting in 74% apparent loading efficiency. Exemplary factors that may affect this percentage include the following. For example, the yield of HPNP synthesis may be less than 100% resulting in broken HPNPs that cannot be sealed but are still counted as SHPNPs. For example, there may be some enzyme leakage out of the particle during the dilution for silica polycondensation reaction. For example, the access of substrate to enzyme may be limited by diffusion of substrate through the porous shell. For example, the enzyme concentration within particles can be adjustable by the concentration of the enzyme solution during the sealing reaction.
[0079] FIG. 16 shows a data plot
1600 showing a standard curve of
Renilla reniformis luciferase activity. Luminescence intensity produced as a result of interaction with benzyl-coelenterazine represents the vertical axis of the data plot
1600.
[0080] FIG. 17 shows a data plot
1700 showing activity plots of different concentrations of
Renilla reniformis luciferase compared to
R. reniformis luciferase encapsulated within sealed hollow porous nanoparticles with a concentration of 1.42×10
12 particles/mL. For example, each reaction was 100 µL in total containing 10 µg/mL benzyl-coelenterazine as substrate. The data plot
1700 shows
Renilla reniformis luciferase activity for concentrations including 0.0008 mg/mL (curve
1701), 0.0004 mg/mL (curve
1702), 0.0002 mg/mL (curve
1703), 0.0001 mg/mL (curve
1704), and 0 mg/mL (curve
1705), and shows 1.42×10
12 SHPNPs/mL (curve
1706).
[0081] The disclosed SHPNPs demonstrate a platform for encapsulating functional biomolecules, e.g., such as enzymes, acting on small molecule substrates that can freely diffuse in and out through the SHPNPs' small size pores. The disclosed SHPNPs can be manufactured in large quantities with sizes and characteristics that can be tightly controlled and the enzyme can be kept in a controlled environment protected from any specific or nonspecific interference from other biomolecules. Exemplary implementations of the disclosed SHPNPs demonstrated that encapsulated enzymes maintain their activities and are effectively shielded from antibodies or proteases, e.g., since the pores of the shells are smaller than the antibodies, proteases, or such molecules. Moreover, for example, surface modifications of SHPNPs can enhance circulation and targeting
in vivo, e.g., without the need of any modification on the encapsulated payload. The disclosed technology provides flexible fabrication techniques of the described SHPNPs with control of particle dimensions and permeability, and the disclosed SHPNPs can be tailored and optimized for specific loads and substrates.
[0082] In another aspect, the disclosed technology can include fabrication protocols for fabricating the metallic nanoparticles with hollow core, porous surface and sealable holes. FIGS. 18A and 18B show schematic diagrams illustrating one exemplary metallic nanoparticle synthesis protocol.
[0083] FIG. 18A shows a process
1820 of binding masking particles
1815 having a functionalized surface
1816 (e.g., a carboxylated surface) to a functionalized surface
1812 (e.g., an aminated surface) of a template core particle
1811, e.g., by electrostatic attraction. For example, since the exemplary carboxylated particles
1815 have a negatively charged surface, they repel negative ions and prevent sol-gel reaction on their surface, e.g., blocking some positively charged regions of the outer surface of the exemplary aminated template particle
1811.
[0084] FIG. 18A shows a process
1830 of adding a colloidal metallic layer
1831 (e.g., colloidal gold) to the masking particles
1815 - template core particle
1811 complex. For example, sol-gel reagents can be added to the solutions containing the masking particles bound to the template particles. The exemplary sol-gel reactions can occur in the positively charged regions along the surface
1812 of the template core particle
1811, e.g., the regions that are not covered or blocked by the masking particles
1815, forming the exemplary colloidal gold layer
1831.
[0085] FIG. 18A shows a process
1840 of thickening the initial layer
1831 into a thick layer 1841. For example, the initial layer
1831 can be formed from colloidal gold generated through sol-gel reactions in the process
1830. The exemplary colloidal gold layer
1831 can act as a nucleation site for further growth of gold, e.g., forming the thick layer
1841. For example, the process
1840 can include the addition of auric acid and formaldehyde as reducing agent for the formation of the exemplary thick gold layer
1841.
[0086] FIG. 18A shows a process
1850 showing forming a hollow porous nanoparticle, e.g., by removing the template particle
1811 and the masking particles
1815. For example, once the layer
1841 is formed with the desired thickness, the template and masking particles are removed, e.g., by various methods including dissolving them by solvents, calcination, melting, or burning, or a combination of these or other similar methods. For example, implementation of the process
1850 yields a metallic HPNP (e.g., a gold HPNP) that includes empty or hollowed porous shell
1841 with holes
1855 and an empty or hollowed interior
1852.
[0087] Once the exemplary metallic HPNPs are created, they can be loaded with other substances and sealed to encapsulate the other substances, e.g., by implementing methods previously described and illustrated in FIGS. 1B and 1C. For example, FIG. 18B shows a process
1860 of loading load particles
1861 into the hollow interior region
1852 of the metallic HPNP
1841. For example, a solution of metallic HPNPs can be loaded with the load substances by adding a high concentration solution of the load substances to the solution of the metallic HPNPs. The process
1860 can be implemented by one of several methods. In one example, the load particles
1861 can diffuse into the metallic HPNPs
1841 through the holes
1855. In other examples, the load particles
1861 can enter the interior region
1852 of the metallic HPNPs
1841 through their holes
1855 by non-diffusion means, e.g., including electrophoretic forces. The process
1860 can be implemented using various types of materials as the load, e.g., including, but not limited to, drugs, biodegradable macromolecules, pH sensitive molecules, enzymes and/or other proteins, lipids, metals, polymers, and ceramic particles, for various applications. For example, subsequent to implementation of the process
1860, the metallic HPNPs
1841 can be sealed to form sealed metallic HPNPs (metallic SHPNPs), e.g., by implementing the process
170 previously described and shown in the FIG. 1C. FIG. 18C shows an image
1890 showing after an exemplary gold HPNP before 500 nm aliphatic-amine polystyrene core extraction.
[0088] In another aspect, the disclosed technology can include fabrication protocols for fabricating the nanoparticles having one or more interior particles within a hollow core, porous surface and sealable holes. FIG. 19 shows schematic diagrams illustrating one exemplary nanoparticle synthesis protocol.
[0089] FIG. 19 shows a process
1920 of binding masking particles
1915 having a functionalized surface
1916 (e.g., a carboxylated surface) to a functionalized surface
1912 (e.g., an aminated surface) of a template core particle
1911, the template particle
1911 having at least one interior particle
1913. For example, the template particle
1911 can be an outer coating of the at least one interior particle
1913 or the template particle
1911 can be a hollow particle that encloses the least one interior particle
1913 within its hollow interior. For example, the process
1920 can include binding the masking particles
1915 to the surface
1912 of the template particle
1911 by electrostatic interactions or means, e.g., including, but not limited to, hydrogen bonding, covalent bonding, magnetic attraction, hydrophobic interactions, etc. For example, since the exemplary carboxylated particles
1915 have a negatively charged surface, they repel negative ions and prevent sol-gel reaction on their surface, e.g., blocking some positively charged regions of the outer surface of the exemplary aminated template particle
1911.
[0090] FIG. 19 shows a process
1930 of adding a layer
1931 (e.g., silica) to the masking particles
1915 - template core particle
1911 complex. For example, sol-gel reagents can be added to the solutions containing the masking particles bound to the template particles. The exemplary sol-gel reactions can occur in the positively charged regions along the surface
1912 of the template core particle
1911, e.g., the regions that are not covered or blocked by the masking particles
1915, forming the exemplary layer
1931.
[0091] FIG. 19 shows a process
1940 of forming a hollow porous nanoparticle including the interior particle
1913 within an interior region
1942, e.g., by removing the template particle
1911 and the masking particles
1915. For example, once the layer
1931 is formed with the desired thickness, the template and masking particles are removed, e.g., by various methods including dissolving them by solvents, calcination, melting, or burning, or a combination of these or other similar methods. For example, implementation of the process
1940 yields an HPNP that includes a porous shell
1941 that includes the interior particle
1913 within its hollowed interior region
1942 and holes
1945 distributed throughout the porous shell
1941, e.g., based on the initial location of the bound masking particles
1915 to the template particle
1911.
[0092] Once the exemplary HPNPs including the at least one interior particle are created, they can be loaded with other substances and sealed to encapsulate the other substances, e.g., by implementing methods previously described and illustrated in FIGS. 1B and 1C. For example, FIG. 19 shows a process
1950 of loading load particles
1951 into the hollow interior region
1942 of the HPNP
1941. For example, a solution of the exemplary HPNPs including the enclosed interior particle(s) can be loaded with the load substances by adding a high concentration solution of the load substances to the solution of the exemplary HPNPs. The process
1950 can be implemented by one of several methods. In one example, the load particles
1951 can diffuse into the HPNPs
1941 through the holes
1945. In other examples, the load particles
1951 can enter the interior region
1942 of the HPNPs
1941 through their holes
1945 by non-diffusion means, e.g., including electrophoretic forces. The process
1950 can be implemented using various types of materials as the load, e.g., including, but not limited to, drugs, biodegradable macromolecules, pH sensitive molecules, enzymes and/or other proteins, lipids, metals, polymers, and ceramic particles, for various applications. For example, within the interior region
1942 of the HPNP
1941, the exemplary load particles
1951 can interact with the interior particle
1913, e.g., forming a modified interior particle
1955. For example, the exemplary load particles
1951 can conjugate to the exterior surface of the interior particle
1913, or in other examples, the exemplary load particles
1951 can chemically react with the interior particle
1913. For example, the modified interior particle
1955 may exhibit new properties otherwise not available on the interior particle
1913.
[0093] In another aspect, the disclosed technology can include fabrication protocols for fabricating the nanoparticles having one hole with a hollow core, e.g., in which the hole can be sealable. FIG. 20 show schematic diagrams illustrating one exemplary nanoparticle synthesis protocol.
[0094] FIG. 20 shows an example of a process
2010 in which a large masking particle
2015 is mixed together with a core template particles
2011. For example, the large masking particle
2015 can be a nanoparticle configured to have a surface charge, e.g., a negative surface charge. Also, for example, the large masking particle
2015 can include particles with a functionalized external surface
2016, e.g., having a surface charge. For example, the exemplary masking particle
2015 can be a polystyrene nanoparticle, and the exemplary functionalized surface
2016 can be a carboxylated-functional layer. For example, the template particle
2011 can be a nanoparticle configured to have a surface charge, e.g., a positive surface charge, of opposite polarity to the surface charge of the masking particle
2015. Also, for example, the template particle
2011 can include a particle with a functionalized external surface
2012. For example, the exemplary template particle
2011 can be a polystyrene nanoparticle, and the exemplary functionalized surface
2012 can be an amine-functional layer. For example, once the exemplary carboxylated masking particle
2015 and aminated template particle
2011 are mixed, the carboxylated particles
2015 can bind to the aminated template particle
2011.
[0095] FIG. 20 also shows an example of a process
2020 of binding of the large masking particle
2015 with the carboxylated functionalized surface
2016 to the aminated functionalized surface
2012 of the template particle
2011, e.g., by electrostatic interactions. In other examples, the process
2020 can include binding the large masking particle
2015 to the surface
2012 of the template particle
2011 by other particle attraction means, e.g., including, but not limited to, hydrogen bonding, covalent bonding, magnetic attraction, hydrophobic interactions, etc.
[0096] FIG. 20 further shows an example of a process
2030 of adding a layer
2031 to the template particle
2011. For example, sol-gel reagents can be added to the solutions containing the masking particle
2015 bound to the template particles
2011. Exemplary sol-gel reactions can occur only in the positively charged regions along the surface
2012 of the template particle
2011, e.g., the region that is not covered or blocked by the masking particle
2015. For example, the process
2030 can cover the exposed surface of the template particle
2011 with the coating
2031 while not covering location where the masking particle
2015 is present. For example, the coating
2031 can be a porous material. For example, the layer
2031 can be of a material (e.g., silica) such that the process
2030 can result in a porous layer forming on the surface of the template particle
2011. For example, addition of sol-gel reactants in the process
2030 can initiate silica growth, e.g., rooted from the amino groups of the exemplary aminated functionalized surface
2012. Also for examples, the coating
2031 can be a non-porous material. In some examples, the process
2030 can include adding the layer
2031 to the template particle
2011 by other means, e.g., including, but not limited to, material based exclusivity, or redox chemistry that forms the layer
2031 only on the surface of one particle (e.g., the template particle
2011) and not the surface of the other particle(s) (e.g., the masking particle
2015), among other techniques. Exemplary materials used for the coating can include porous or non-porous materials, or degradable materials (e.g., that can dissolve or degrade in certain environments or under particular conditions or by an exemplary trigger, e.g., conditions and/or trigger including pH, temperature, pressure, molecular interaction, or other conditions and/or triggers).
[0097] In addition, FIG. 20 shows an example of a process
2040 of forming a hollow nanoparticle, e.g., by removing the template particle
2011 and the masking particle
2015. For example, once the layer
2031 is formed with the desired thickness, the template particle
2011 and masking particle
2015 are removed, e.g., by various methods including dissolving them by solvents, calcination, melting, or burning, or a combination of these or other similar methods. For example, implementation of the process
2040 yields a hollow nanoparticle that include an empty or hollowed porous shell
2041 with a hole
2045 and a hollowed interior
2042. In some examples, the process
2040 can be implemented to form a hollow non-porous nanoparticle, e.g., when the layer
2031 is of a porous material. In other examples, the process
2040 can be implemented to form a hollow non-porous nanoparticle, e.g., when the layer
2031 is of a non-porous material. Once the exemplary hollow shell structure is formed, it can be loaded with other substances and sealed to encapsulate the other substances, e.g., by implementing methods previously described and illustrated in FIGS. 1B and 1C.
[0098] Applications of the described nanoparticle platform can include at least the following. Macromolecules larger than the pores can be diffused inside the nanoparticle through holes on the surface and later can be released gradually. Once the macromolecules diffuse inside the nanoparticle through holes, holes are sealed. Since the particle surface is porous, small molecules can diffuse in and outside therefore providing communication of the macromolecule with the outside environment while protecting either the environment from macromolecules or protecting the macromolecules from environment. For example, macromolecule inside the particle can be used as a sensor reporting some event in the environment without being exposed to the environment. For example, once the macromolecules diffused inside the particle, the holes can be sealed with molecules having a particular property (e.g., such as a degradation property). For example, the particular property can be exploited, and the macromolecules encapsulated in the particle can be released. For example, the macromolecules sealed inside the HPNP can include a particular property such as reacting with a molecule small enough to pass through the pores. For example, the macromolecule might be an enzyme molecule used to activate a small drug molecule. Since the exemplary enzyme molecule is encapsulated inside the particle, it is hidden from the immune system. For example, the surface of HPNPs can be functionalized with targeting agents, e.g., for efficient deployment and delivery to the target region. For example, an inactivated drug can be introduced to the circulation separately. Since the exemplary drug is not activated, the drug is not dose limited. For example, once the exemplary inactivated drug and enzyme-loaded HPNP meet in the target region of the body, the drug can diffuse inside the HPNP and become activated by the enzyme; and the activated drug can diffuse out of the HPNP to the target region, e.g., thereby affecting only the target region.
[0099] Only a few implementations and examples are described and other implementations, enhancements and variations can be made based on what is described and illustrated as long as they fall within the scope of the claims.